A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons

BACKGROUND: Lack of appropriate tools and techniques to study fate and functional integration of newly generated neurons has so far hindered understanding of neurogenesis' relevance under physiological and pathological conditions. Current analyses are either dependent on mitotic labeling, for e...

Descripción completa

Detalles Bibliográficos
Autores principales: Zhang, Jingzhong, Giesert, Florian, Kloos, Karina, Vogt Weisenhorn, Daniela M, Aigner, Ludwig, Wurst, Wolfgang, Couillard-Despres, Sebastien
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3019205/
https://www.ncbi.nlm.nih.gov/pubmed/21194452
http://dx.doi.org/10.1186/1471-2202-11-158
_version_ 1782196185994362880
author Zhang, Jingzhong
Giesert, Florian
Kloos, Karina
Vogt Weisenhorn, Daniela M
Aigner, Ludwig
Wurst, Wolfgang
Couillard-Despres, Sebastien
author_facet Zhang, Jingzhong
Giesert, Florian
Kloos, Karina
Vogt Weisenhorn, Daniela M
Aigner, Ludwig
Wurst, Wolfgang
Couillard-Despres, Sebastien
author_sort Zhang, Jingzhong
collection PubMed
description BACKGROUND: Lack of appropriate tools and techniques to study fate and functional integration of newly generated neurons has so far hindered understanding of neurogenesis' relevance under physiological and pathological conditions. Current analyses are either dependent on mitotic labeling, for example BrdU-incorporation or retroviral infection, or on the detection of transient immature neuronal markers. Here, we report a transgenic mouse model (DCX-CreERT2) for time-resolved fate analysis of newly generated neurons. This model is based on the expression of a tamoxifen-inducible Cre recombinase under the control of a doublecortin (DCX) promoter, which is specific for immature neuronal cells in the CNS. RESULTS: In the DCX-CreERT2 transgenic mice, expression of CreERT2 was restricted to DCX+ cells. In the CNS of transgenic embryos and adult DCX-CreERT2 mice, tamoxifen administration caused the transient translocation of CreERT2 to the nucleus, allowing for the recombination of loxP-flanked sequences. In our system, tamoxifen administration at E14.5 resulted in reporter gene activation throughout the developing CNS of transgenic embryos. In the adult CNS, neurogenic regions were the primary sites of tamoxifen-induced reporter gene activation. In addition, reporter expression could also be detected outside of neurogenic regions in cells physiologically expressing DCX (e.g. piriform cortex, corpus callosum, hypothalamus). Four weeks after recombination, the vast majority of reporter-expressing cells were found to co-express NeuN, revealing the neuronal fate of DCX+ cells upon maturation. CONCLUSIONS: This first validation demonstrates that our new DCX-CreERT2 transgenic mouse model constitutes a powerful tool to investigate neurogenesis, migration and their long-term fate of neuronal precursors. Moreover, it allows for a targeted activation or deletion of specific genes in neuronal precursors and will thereby contribute to unravel the molecular mechanisms controlling neurogenesis.
format Text
id pubmed-3019205
institution National Center for Biotechnology Information
language English
publishDate 2010
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-30192052011-01-12 A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons Zhang, Jingzhong Giesert, Florian Kloos, Karina Vogt Weisenhorn, Daniela M Aigner, Ludwig Wurst, Wolfgang Couillard-Despres, Sebastien BMC Neurosci Research Article BACKGROUND: Lack of appropriate tools and techniques to study fate and functional integration of newly generated neurons has so far hindered understanding of neurogenesis' relevance under physiological and pathological conditions. Current analyses are either dependent on mitotic labeling, for example BrdU-incorporation or retroviral infection, or on the detection of transient immature neuronal markers. Here, we report a transgenic mouse model (DCX-CreERT2) for time-resolved fate analysis of newly generated neurons. This model is based on the expression of a tamoxifen-inducible Cre recombinase under the control of a doublecortin (DCX) promoter, which is specific for immature neuronal cells in the CNS. RESULTS: In the DCX-CreERT2 transgenic mice, expression of CreERT2 was restricted to DCX+ cells. In the CNS of transgenic embryos and adult DCX-CreERT2 mice, tamoxifen administration caused the transient translocation of CreERT2 to the nucleus, allowing for the recombination of loxP-flanked sequences. In our system, tamoxifen administration at E14.5 resulted in reporter gene activation throughout the developing CNS of transgenic embryos. In the adult CNS, neurogenic regions were the primary sites of tamoxifen-induced reporter gene activation. In addition, reporter expression could also be detected outside of neurogenic regions in cells physiologically expressing DCX (e.g. piriform cortex, corpus callosum, hypothalamus). Four weeks after recombination, the vast majority of reporter-expressing cells were found to co-express NeuN, revealing the neuronal fate of DCX+ cells upon maturation. CONCLUSIONS: This first validation demonstrates that our new DCX-CreERT2 transgenic mouse model constitutes a powerful tool to investigate neurogenesis, migration and their long-term fate of neuronal precursors. Moreover, it allows for a targeted activation or deletion of specific genes in neuronal precursors and will thereby contribute to unravel the molecular mechanisms controlling neurogenesis. BioMed Central 2010-12-31 /pmc/articles/PMC3019205/ /pubmed/21194452 http://dx.doi.org/10.1186/1471-2202-11-158 Text en Copyright ©2010 Zhang et al; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (<url>http://creativecommons.org/licenses/by/2.0</url>), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Zhang, Jingzhong
Giesert, Florian
Kloos, Karina
Vogt Weisenhorn, Daniela M
Aigner, Ludwig
Wurst, Wolfgang
Couillard-Despres, Sebastien
A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title_full A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title_fullStr A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title_full_unstemmed A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title_short A powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
title_sort powerful transgenic tool for fate mapping and functional analysis of newly generated neurons
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3019205/
https://www.ncbi.nlm.nih.gov/pubmed/21194452
http://dx.doi.org/10.1186/1471-2202-11-158
work_keys_str_mv AT zhangjingzhong apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT giesertflorian apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT klooskarina apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT vogtweisenhorndanielam apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT aignerludwig apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT wurstwolfgang apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT couillarddespressebastien apowerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT zhangjingzhong powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT giesertflorian powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT klooskarina powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT vogtweisenhorndanielam powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT aignerludwig powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT wurstwolfgang powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons
AT couillarddespressebastien powerfultransgenictoolforfatemappingandfunctionalanalysisofnewlygeneratedneurons

Ejemplares similares